Team:SDU-Denmark/protocols

From 2010.igem.org

(Difference between revisions)
(Extraction af Carotenoids and polyene chromophores)
(Protocols)
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3. Re-suspend cells in 8 mL acetone and sonicate the sample for 2x 2 min<br>  
3. Re-suspend cells in 8 mL acetone and sonicate the sample for 2x 2 min<br>  
4. Centrifuge the samples at 16000 G for 2 min and collect the supernatant<br>
4. Centrifuge the samples at 16000 G for 2 min and collect the supernatant<br>
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5. Measure absorbance using an HPLC at 450 nm using a C18… column with 50% Acetonitrill, 50% water and 10% Acetonitrill 90% Methanol as eluents A and B <br>
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5. Measure absorbance using an HPLC at 450 nm using a C18… column with 50% Acetonitrill, 50% water and 10% Acetonitrill 90% Methanol as eluents A and B <br><br>
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==Photosensor characterisation==
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===PS1.1===
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''Materials''<br>
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• Diluted LB media<br>
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• Difco Agar<br>
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• 1mM retinal<br><br>
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''Swimming motility plates''<br>
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1. LB media is mixed with 0.3% difco agar and is autoclavated<br>
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2. The appropriate antibiotic and 1uM retinal is added to the autoclaved media (NB: for the media used for the control plates, no antibiotic or retinal is added)<br>
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3. Plates are cast and incubated ON at room temperature<br>
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4. 15 minutes prior to the experiment the plates are incubated at 37°C.<br><br>
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''Sample preparation''<br>
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1. Colony is inoculated in 5mL LB media containing the appropriate antibiotic. The culture is grown ON at 37°C and 180rpm.<br>
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2. ON culture is diluted in 5mL LB media containing the appropriate antibiotic to reach an OD550 of 0.02 and are incubated at 37°C and 180rpm until it reaches an OD550 of 0.5.<br>
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3. 1mM retinal is added to the culture (NB: no retinal is added to the cultures containing the control cells)<br>
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4. The tubes containing the cultures are wrapped in tin foil and are subsequently grown for 2 hours at 37°C and 180rpm.<br><br>
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''Motility assay''<br>
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1. 2x2.5uL of culture is placed on each plate, and the plates are placed in a specially engineered lightbox, so that ½ of each plate is illuminated with blue light and the other ½ is kept in dark. 1mL of each culture is used for microscopy.<br>
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2. The plates are incubated at 37°C for 24 hours.<br>
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3. Pictures are taken<br><br>
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''Microscopy''<br>
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1. 5uL cell culture is used for the microscopy<br>
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2. To avoid laminar flow, the microscopy slide is sealed with nail polish.<br>
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3. Samples are examined under the microscope.<br><br>
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==Growth rate assay==
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===GA1.1===
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''Materials''<br>
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• LB media<br>
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• Spectrophotometer<br><br>
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''Protocol''<br>
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1. A colony is inoculated in 5mL LB media containing the appropriate antibiotic.<br>
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2. The culture is incubated over night at 37°C and 180rpm.<br>
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3. The optical density at 550nm (OD550) of the ON culture is measured and the culture is diluted in 25uL fresh LB media containing the appropriate antibiotic to reach an OD550 of 0.02. The culture is incubated for 24 hours at 37°C and 180rpm.<br>
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4. OD550 of the colony is measured every hour for the first 12 hours, and after 24 hours.<br><br>
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Revision as of 11:47, 18 October 2010